Microfluidic tectonics: A comprehensive construction platform for microfluidic systems

Beebe, David J.; Moore, Jeffrey S.; Yu, Qing; Liu, Robin H.; Kraft, Mary L.; Jo, Byung Ho; Devadoss, Chelladurai

doi:10.1073/pnas.250273097

Cited by 339 publications

(266 citation statements)

References 8 publications

Supporting

Mentioning

262

Contrasting

Order By: Relevance

“…Numerous techniques exist for creation of constructs as cell-supportive matrices, including electrospinning 13 , elastomer stamps 14 , inkjet printing 15 , additive photopatterning 16 , static photomask projection-lithography 17 , and dynamic mask microstereolithography 18 . Unfortunately, these methods involve multiple production steps and/or equipment not readily adaptable to conventional cell and tissue culture methods.…”

mentioning

confidence: 99%

Fabrication of Micropatterned Hydrogels for Neural Culture Systems using Dynamic Mask Projection Photolithography

Curley

Jennings

Moore

2011

JoVE

View full text Add to dashboard Cite

Increasingly, patterned cell culture environments are becoming a relevant technique to study cellular characteristics, and many researchers believe in the need for 3D environments to represent in vitro experiments which better mimic in vivo qualities [1][2][3] . Studies in fields such as cancer research , and cell-matrix interaction 7,8 have shown cell behavior differs substantially between traditional monolayer cultures and 3D constructs.Hydrogels are used as 3D environments because of their variety, versatility and ability to tailor molecular composition through functionalization [9][10][11][12] . Numerous techniques exist for creation of constructs as cell-supportive matrices, including electrospinning . Unfortunately, these methods involve multiple production steps and/or equipment not readily adaptable to conventional cell and tissue culture methods. The technique employed in this protocol adapts the latter two methods, using a digital micromirror device (DMD) to create dynamic photomasks for crosslinking geometrically specific poly-(ethylene glycol) (PEG) hydrogels, induced through UV initiated free radical polymerization. The resulting "2.5D" structures provide a constrained 3D environment for neural growth. We employ a dual-hydrogel approach, where PEG serves as a cellrestrictive region supplying structure to an otherwise shapeless but cell-permissive self-assembling gel made from either Puramatrix or agarose. The process is a quick simple one step fabrication which is highly reproducible and easily adapted for use with conventional cell culture methods and substrates.Whole tissue explants, such as embryonic dorsal root ganglia (DRG), can be incorporated into the dual hydrogel constructs for experimental assays such as neurite outgrowth. Additionally, dissociated cells can be encapsulated in the photocrosslinkable or self polymerizing hydrogel, or selectively adhered to the permeable support membrane using cell-restrictive photopatterning. Using the DMD, we created hydrogel constructs up to ~1mm thick, but thin film (<200 μm) PEG structures were limited by oxygen quenching of the free radical polymerization reaction. We subsequently developed a technique utilizing a layer of oil above the polymerization liquid which allowed thin PEG structure polymerization.In this protocol, we describe the expeditious creation of 3D hydrogel systems for production of microfabricated neural cell and tissue cultures. The dual hydrogel constructs demonstrated herein represent versatile in vitro models that may prove useful for studies in neuroscience involving cell survival, migration, and/or neurite growth and guidance. Moreover, as the protocol can work for many types of hydrogels and cells, the potential applications are both varied and vast. Video LinkThe video component of this article can be found at https://www.jove.com/video/2636/ Protocol 1. DMD Setup 1. The DMD board, UV light guide (with collimator) and 4x objective lens are all mounted vertically on a vibration isolation table. 2. The UV light guide sh...

show abstract

mentioning

confidence: 99%

Fabrication of Micropatterned Hydrogels for Neural Culture Systems using Dynamic Mask Projection Photolithography

Curley

Jennings

Moore

2011

JoVE

View full text Add to dashboard Cite

show abstract

“…F luid mechanics on the micrometer scale has enjoyed much attention recently, not only because of the desire to incorporate fluids devices such as pumps or valves into microelectromechanical systems (1,2), but also because of the potential applications in biomedicine and bioengineering. The flow of liquid in these devices is regulated by a large variety of applied forces (3), such as pressure differences, electrophoresis (4), capillary forces (5), or Marangoni forces (6).…”

mentioning

confidence: 99%

A bubble-driven microfluidic transport element for bioengineering

Marmottant

Hilgenfeldt

2004

Proc. Natl. Acad. Sci. U.S.A.

170

158

View full text Add to dashboard Cite

Microfluidics typically uses channels to transport small objects by actuation forces such as an applied pressure difference or thermocapillarity. We propose that acoustic streaming is an alternative means of directional transport at small scales. Microbubbles on a substrate establish well controlled fluid motion on very small scales; combinations (''doublets'') of bubbles and microparticles break the symmetry of the motion and constitute flow transport elements. We demonstrate the principle of doublet streaming and describe the ensuing transport. Devices based on doublet flow elements work without microchannels and are thus potentially cheap and highly parallelizable.

show abstract

“…[18][19][20]23,24,46,94 The swelling property of hydrogels allows integration of actuators such as valves, allowing integration of sophisticated fluid handling functions. 133 A wide range of immobilization methods are available to hydrogels, including copolymerization of proteins, 18,19,23,94,132 activation for covalent linking of proteins, 134 or electrostatic capture on charged hydrogel. 20,24 Even with a 3-D microchannel-filling hydrogel, the microchannel surface should be functionalized for covalent anchoring of the hydrogel structure within the channel, so that the gel will not drift out of the channel under hydrodynamic pressure or applied electric field.…”

Section: Hydrogelmentioning

confidence: 99%

“…82,83 The microfluidic-chip fabrication process is rather interesting in that the authors fabricated a microfluidic channel using in situ polymerization of the monomer isobornyl acrylate (IBA) in an empty chamber made of a bottom glass slide, a polycarbonate top, and an intermediate adhesive rim, whereas typical microfluidic chip fabrication is done by etching bulk material. 133 After the glass slide was silanized with (3-acryloxypropyl)-trimethoxysilane to provide an acryloyl group, macroporous PEG pillars were photopolymerized using PEGDA monomer. PEG porogens of various molecular masses were used to form macropores.…”

Section: Amine-nhs (N-hydroxysuccinimide)mentioning

confidence: 99%

Protein immobilization techniques for microfluidic assays

2013

View full text Add to dashboard Cite

Microfluidic systems have shown unequivocal performance improvements over conventional bench-top assays across a range of performance metrics. For example, specific advances have been made in reagent consumption, throughput, integration of multiple assay steps, assay automation, and multiplexing capability. For heterogeneous systems, controlled immobilization of reactants is essential for reliable, sensitive detection of analytes. In most cases, protein immobilization densities are maximized, while native activity and conformation are maintained. Immobilization methods and chemistries vary significantly depending on immobilization surface, protein properties, and specific assay goals. In this review, we present trade-offs considerations for common immobilization surface materials. We overview immobilization methods and chemistries, and discuss studies exemplar of key approaches—here with a specific emphasis on immunoassays and enzymatic reactors. Recent “smart immobilization” methods including the use of light, electrochemical, thermal, and chemical stimuli to attach and detach proteins on demand with precise spatial control are highlighted. Spatially encoded protein immobilization using DNA hybridization for multiplexed assays and reversible protein immobilization surfaces for repeatable assay are introduced as immobilization methods. We also describe multifunctional surface coatings that can perform tasks that were, until recently, relegated to multiple functional coatings. We consider the microfluidics literature from 1997 to present and close with a perspective on future approaches to protein immobilization.

show abstract

Microfluidic tectonics: A comprehensive construction platform for microfluidic systems

Cited by 339 publications

References 8 publications

Fabrication of Micropatterned Hydrogels for Neural Culture Systems using Dynamic Mask Projection Photolithography

Fabrication of Micropatterned Hydrogels for Neural Culture Systems using Dynamic Mask Projection Photolithography

A bubble-driven microfluidic transport element for bioengineering

Protein immobilization techniques for microfluidic assays

Contact Info

Product

Resources

About